Method for preparation of carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl ester

ABSTRACT

Disclosed is a method for the preparation of carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl esters, comprising the enantioselective enzyme reduction of a 1-aryl-2-tetrazolyl-ethyl ketone to form a (R)-1-aryl-2-tetrazolyl-ethyl alcohol and the carbamation of said alcohol.

CROSS-REFERENCE TO RELATED APPLICATIONS

This application is a continuation of U.S. application Ser. No. 13/776,964, filed on Feb. 26, 2013, which is a divisional application of U.S. application Ser. No. 12/904,267, filed on Oct. 14, 2010, issued as U.S. Pat. No. 8,404,461, on Mar. 26, 2013, which claims the benefit and priority to U.S. Provisional Application Ser. No. 61/251,867, filed Oct. 15, 2009. The entire disclosures of the applications identified in this paragraph are incorporated herein by references.

The present invention relates to a method for the preparation of carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl ester. More particularly, the present invention relates to a method for preparing carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl ester, comprising the enantioselective enzyme reduction of an arylketone.

BACKGROUND OF THE INVENTION

As disclosed in U.S. Patent Application Publication No. 2006/0258718 A1, carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl esters (hereinafter referred to as “the carbamate compounds”) possess anticonvulsant activity and are useful in the treatment of disorders of the central nervous system, especially including anxiety, depression, convulsion, epilepsy, migraines, bipolar disorder, drug abuse, smoking, ADHD, obesity, sleep disorders, neuropathic pain, strokes, cognitive impairment, neurodegeneration, strokes and muscle spasms.

Depending on the position of N in the tetrazole moiety thereof, the carbamate compounds are divided into two positional isomers: tetrazole-1-yl (hereinafter referred to as “1N tetrazole”) and treatzole-2-yl (hereinafter referred to as “2N tetrazole”). The introduction of tetrazole for the preparation of the carbamate compounds results in a 1:1 mixture of the two positional isomers which are required to be individually isolated for pharmaceutical use.

Having chirality, the carbamate compounds must be in high optical purity as well as chemical purity as they are used as medications. In this regard, U.S. Patent Application Publication No. 2006/0258718 A1 uses the pure enantiomer (R)-aryl-oxirane as a starting material, which is converted into an alcohol intermediate through a ring-opening reaction by tetrazole in the presence of a suitable base in a solvent, followed by introducing a carbamoyl group into the resulting alcohol intermediate. For isolation and purification of the 1N and 2N positional isomers thus produced, column chromatography is utilized after the formation of an alcohol intermediate or carbamate.

For use in the preparation described above, (R)-2-aryl-oxirane may be synthesized from an optically active material, such as substituted (R)-mandelic acid derivative via various route, or obtained by asymmetric reduction-ring formation reaction of α-halo arylketone, or by separation of racemic 2-aryl-oxirane mixture into its individual enantiomers. As such, (R)-2-aryl-oxirane is an expensive compound.

In addition, the ring-opening reaction of (R)-2-aryl-oxirane with tetrazole is performed at relatively high temperatures because of the low nucleophilicity of the tetrazole. However, because tetrazoles start to spontaneously degrade at 110˜120° C., the ring opening reaction includes the highly likely risk of a runaway reaction.

In terms of a selection of reaction, as there are two reaction sites in each (R)-2-aryl-oxirane and tetrazole, the ring-opening reaction therebetween affords the substitution of 1N- or 2N-tetrazole at the benzyl or terminal position, resulting in a mixture of a total of 4 positional isomers. Therefore, individual positional isomers are low in production yield and difficult to isolate and purify.

SUMMARY OF THE INVENTION

In accordance with the present invention, the foregoing disadvantages of the prior art are overcome by a novel method for preparing carbamic (R)-1-aryl-2-tetrazolyl-ethyl esters. In the present method, a (R)-1-aryl-2-tetrazolyl-ethyl alcohol represented by Chemical Formula 3 is formed by the enantioselective enzymatic reduction of an arylketone, represented by Chemical Formula 2, and the alcohol is then carbamated to form the carbamic acid (R)-1-aryl-2-tetrazolyl ethyl ester, represented by Chemical Formula 1:

wherein, R₁ and R₂ are independently selected from a group consisting of hydrogen, halogen, perfluoroalkyl, alkyl of 1 to 8 carbon atoms, thioalkoxy of 1 to 8 carbon atoms, and alkoxy of 1 to 8 carbon atoms; and one of A₁ and A₂ is CH with the other being N.

DESCRIPTION OF THE PREFERRED EMBODIMENTS

In accordance with an embodiment of the present invention, a method comprising enantioselective enzymatic reduction of an arylketone represented by the following Chemical Formula 2 and the carbamation of the resultant alcohol compound represented by the following Chemical Formula 3 is provided for the preparation of carbamic acid (R)-1-aryl-2-tetrazolyl-ethyl ester, represented by the following Chemical Formula 1.

wherein,

R₁ and R₂ are independently selected from a group consisting of hydrogen, halogen, perfluoroalkyl, alkyl of 1 to 8 carbon atoms, thioalkoxy of 1 to 8 carbon atoms, and alkoxy of 1 to 8 carbon atoms; and

one of A₁ and A₂ is CH with the other being N.

The arylketone of Chemical Formula 2, useful as a starting material in the preparation method of the present invention, may be synthesized by, for example, a substitution reaction between the arylketone of Chemical Formula 4 and tetrazole of Chemical Formula 5:

wherein,

R₁ and R₂ are as defined above; and

X is a leaving group, such as a halide or sulfonate.

An economical advantage is given to the synthesis of the arylketones of Chemical Formula 2 from the compounds represented by Chemical Formulae 4 and 5 because they are commercially available, relatively inexpensive compounds. In addition, the substitution reaction can be carried out in relatively mild conditions, compared to the ring-opening reaction between (R)-2-aryl-oxirane and tetrazole. The method according to the present invention is therefore certain of process safety, although employing potentially explosive tetrazole, and ensures high production yield and easy purification, with the production of no unnecessary positional isomers at benzyl positions.

The arylketone represented by Chemical Formula 2 which can be synthesized by the substitution reaction with tetrazole may be in a mixture of positional isomers including 1N arylketone of the following Chemical Formula 2a and 2N arylketone of the following Chemical Formula 2b, which can be isolated and purified through commercially available crystallization.

The crystallization useful in the present invention may comprise adding a solubilizing agent to the product of the substitution reaction, that is a mixture of the positional isomers, and then adding a precipitating agent. Optionally, the crystallization may further comprise, after the precipitation, filtrating the precipitate, concentrating the filtrate and adding an additional precipitating agent.

Illustrative, non-limiting examples of the solubilizing agent include acetone, acetonitrile, tetrahydrofuran, ethyl acetate, dichloromethane, chloroform, 1,4-dioxane, and lower alcohols of 1 to 4 carbon atoms, and combinations thereof. The solubilizing agent may be used in an amount of from 0 to 20 ml (v/w) based on the weight (g) of the mixture of the positional isomers. As used herein, the addition of the solubilizing agent in an amount of zero ml (v/w) is intended to mean immediately adding the subsequent precipitating agent without dilution of the filtrate.

Examples of the precipitating agent include water, C1-C4 lower alcohol, diethylether, pentane, hexane, cyclohexane, heptane and combinations thereof, but are not limited thereto. The precipitating agent may be slowly added in an amount of from zero to 40 ml (v/w) based on the weight (g) of the mixture of positional isomers. As used herein, the addition of the precipitating agent in an amount of zero ml is intended to mean allowing the reaction mixture to stand, or cooling it without the addition of the precipitating agent to yield the precipitates. Filtration of the precipitates yields the 1N arylketone of Chemical Formula 2a as crystals with high purity.

On the other hand, the filtrate thus obtained after the filtration step may be concentrated to increase the ratio of the precipitating agent to the solubilizing agent, thereby yielding the 2N arylketone of Chemical Formula 2b with high purity. The concentration ratio of the filtrate can be suitably determined by those of ordinary skill in the art. For example, concentration is carried until the solvent is totally removed off, then the solubilizing agent and the precipitating agent are added as described above. Unlike column chromatography, this crystallization may be commercially used without much difficulty.

The enantioselective enzymatic reduction according to the present invention allows for the conversion of the arylketone of Chemical Formula 2 above into the alcohol compound with (R)-configuration, represented by the Chemical Formula 3 above. The enantioselective enzymatic reduction may be performed using an oxidoreductase enzyme that is in suspension in the reaction mixture, or immobilized in a conventional manner. The enzyme may be utilized in a completely purified state, in a partially purified state, or in the microbial cells is which it was expressed. The cells themselves may be in a native state, a permeabilized state or a lysed state. It will be appreciated by those of ordinary skill in the art that use of the enzyme in the cells is preferred for the practice of the process of the invention since it represents a significant savings in cost. Most preferably, the enzyme is expressed in E. coli and used as a suspension of native cells.

The process of enzymatic reduction of the aryl ketone compounds of Formula 2 can be performed in a reaction mixture comprising said compound of Chemical Formula 2, an oxidoreductase, NADH or NADPH as a cofactor, a cosubstrate and a suitable buffer wherein the oxidoreductase comprises an amino acid sequence wherein at least 60% of the amino acids are identical with one of the amino acid sequences SEQ ID NO: 1, SEQ ID NO: 2, SEQ ID NO: 3 or SEQ ID NO:4.

It has been found that polypeptides comprising one of amino acid sequences SEQ ID NO: 1, SEQ ID NO: 2, SEQ ID NO: 3 or SEQ ID NO:4 or a polypeptides comprising an amino sequence which is identical by at least 60%, preferably at least 90% to one of the amino acid sequences SEQ ID NO: 1, SEQ ID NO: 2, SEQ ID NO: 3 or SEQ ID NO:4 and possessing oxidoreductase activity can be used for reducing the compound of Formula 2 to the compound of Formula 3 (R-configuration) with high conversion and high enatiomeric selectivity. The enantiomeric excess of the R-alcohol formed in the enantioselective enzymatic reduction is at least about 89%, preferably at least about 95% and most preferably at least about 99%.

The organism producing the oxidoreductase polypeptides useful in the enantioselective enzymatic reduction may be a wild strain or a variant and is preferably selected from Candida magnolia, Candida vaccinii, and Oryctolagus cuniculus, Yeast of the Candida genus is preferred for producing the oxidoreductase enzymes utilized in the present process. Derivatives of the polypeptides are those having at least sixty percent homology with the SEQ IDs given above and possessing oxidoreductase activity. Those skilled in the art are aware that there are systems and technology available to accurately determine sequence homology.

A polypeptide comprising SEQ ID NO:1 may be encoded by a DNA sequence SEQ ID NO:5 which is obtainable, for example, from the organism Oryetoiagus cuniculus deposited under the conditions of the Budapest Treaty with the Deutsche Sammlung für Mikroorganismen und Zellkulturen, Mascheroder Weg 1b, 38124 under the number DSMZ 22167, specifically from rabbit DSMZ 22167, or by a nucleic acid sequence that hybridizes therewith. A polypeptide comprising SEQ ID NO:2 may be encoded by a DNA sequence SEQ ID NO:6 which is obtainable, for example, from the organism Candida magnoliae DSMZ 22052, or by a nucleic acid sequence that hybridizes therewith.

A polypeptide comprising SEQ ID NO:3 may be encoded by a DNA sequence SEQ ID NO:7, which is obtainable, for example, from the organism Candida vaccinii CBS7318, or by a nucleic acid sequence that hybridizes therewith. A polypeptide comprising SEQ ID NO:4 may be encoded by a DNA sequence SEQ ID NO:8, which is obtainable, for example, from the organism Candida magnoliae CBS6396, or by a nucleic acid sequence that hybridizes therewith.

The oxidoreductase having one of polypeptide sequences mentioned above is obtained in useable quantities by conventional procedures recognized by those skilled in the art. A polynucleotide coding for the amino acid sequence is cloned into a suitable vector and thereafter introduced into a host organism capable of expressing the gene coding for the sequence. Microorganisms susceptible of transforming to become capable of expressing of such a peptide are well known in the art. A preferred microorganism is Escherichia coli. As stated above, the oxidoreductase expressed by transformed E. coli may be extracted from the E. coli cells and partially or completely purified for use in the process, or may be utilized in the cells themselves which may be in a native, permeabilized or lysed state. A preferred embodiment of the enantioselective enzymatic reduction of the present invention utilizes a suspension of the oxidoreductase as cells in the native state. Any of these forms may be utilized in the free or immobilized form.

The reduction reaction may be carried out in a single phase system having the cells containing the enzyme suspended therein. Alternatively, the reaction may be performed in a two-phase aqueous/organic solvent system as described in U.S. Patent Application Publication No. 2009/0017510 and U.S. Pat. No. 7,371,903. The reaction may be carried out as a conventional batch reaction, or as a continuous process. It will be appreciated that one of the significant advantages of the enantioselective enzymatic reduction for commercial applications is that it is amenable to continuous operation.

The reaction mixture preferably contains from about 35 g to 350 g of cells per kg of reactant added therein. The suspension is the aqueous portion of the reaction mixture which also contains a buffer, for example a TEA (triethanolamine), phosphate, Tris/HCl or glycine buffer. The buffer may additionally comprise ions for the stabilization of the enzyme, for example, a source of magnesium ions. Additional additives that may be present in the buffer for stabilizing the enzymes may include a polyol such as glycerol, sorbitols and the like, sulfur compounds, such as 1,4DL-dithiothreitol, glutathione, cysteine or the like, amino acids and peptides, or detergents, such as DMSO. A preferred stabilizer for the enzyme is a polyol, particularly glycerol, which may be present in from about 10% to 80% by weight, preferably about 50% by weight, based on the weight of the cell suspension.

The enantioselective enzymatic reduction process is advantageously carried out using a coupled substrate principle wherein the reaction mixture utilizes a cosubstrate for the regeneration of the cofactor, or coenzyme, which functions to provide hydrogen for the reduction of the arylketone substrate. The cofactor is preferably nicotineamide adenine dinucleotide phosphate (NADP) or nicotineamide adenine dinucleotide (NAD), which are utilized in the reduced state, i.e. NADPH or NADH, respectively. The cofactor is present in the reaction mixture in a concentration of from about 0.01 mM to 5 mM, preferably 0.05 mM to 0.5 mM. In the reaction, the cosubstrate functions by being oxidized in the regeneration of the NADPH or NADH cofactor. The cosubstrate is a secondary alcohol represented by the Formula R_(x)R_(y)CHOH, wherein R_(x) represents carbon with x being an integer from 1-10 and R_(y) represents hydrogen with y being an integer equal to two times the value of x plus two. Examples of suitable cosubstrates include 2-propanol, 2-butanol 4-methyl-2-pentanol, 2-pentanol, 2-heptanol, 2-octanol and the like. A preferred cosubstrate is 2-butanol. The cosubstrate is present in the reaction mixture in from about 10% to 80% by volume, preferably from about 40% to 60% by volume, most preferably about 50% by volume.

The oxidized cofactor formed during the reduction of the arylketone is regenerated by oxidation of the cosubstrate, which also can be catalyzed by the oxidoreductase. Thus, a particular economic advantage of the present process is that the oxidoreductase affects both reduction of the arylketone of Formula 1 and oxidation of the cosubstrate, therefore no further enzyme has to be used for cofactor regeneration. It is also within the scope of the present invention to add another enzyme to the reaction mixture for cofactor regeneration in order to enhance the rate of reduction of the aryl ketone.

In a further embodiment, an organic solvent that is not involved in the regeneration of the cofactor may be added to the reaction mixture and the reduction process carried out in an aqueous organic 2-phase system. Examples of such solvents include, without intended limitation, diethyl ether, tertiary butyl methyl ether, diisopropyl ether, dibutyl ether, ethyl acetate, butyl acetate, heptane, hexane or cyclohexane. Such a solvent may be present in from about 1% to 50% by volume based on the volume of the reaction mixture.

The amount of the arylketone substrate in the reaction mixture is preferably greater than about 0.1% by weight and may be increased to about 50% by weight, with a preferred concentration being from about 5 to 30% by weight. The amount of the substrate will vary depending on the purity thereof since the process may be carried out with the substrate in a purified state or as raw product containing varying amounts and types of impurities. The pH of the reaction mixture after the addition of all components will be in the range of 5 to 10, preferably from 7 to 9, and optimally about pH 8. The enzymatic reduction according to the present invention is carried out at a temperature of from about 10-45° C., preferably from about 20-40° C., most preferably from about 25-35° C.

The enantioselective reduction process is cost-effective and environment-friendly in addition to providing the alcohols of Formula 3 in high yield and very high enantioselectivity. Thus, an alcohol compound with an (R)-configuration of high optical purity can be obtained in the presence of the enzyme under the above-mentioned reaction conditions within, from about 12 to 96 hours, preferably from about 24 to 48 hours. During the incubation, the pH of the mixture is maintained within the ranges given above by periodic testing and the addition of a conventional acidic or basic reagents, for example sodium carbonate and sodium hydroxide, respectively. The efficiency of the enantioselective enzymatic reduction can be expressed by the total turnover number (TTN) which is the moles of the chiral alcohol of Formula 2 produced per mole of cofactor used. The TTN of the enantioselective enzymatic reduction is from about 10² to 10⁵, preferably ≧10³.

When the alcohol compound obtained through the enantioselective enzymatic reduction exists as a positional isomer mixture of 1N alcohol of Chemical Formula 3a and 2N alcohol of Chemical Formula 3b, it can be isolated and purified into individual positional isomers of high purity by crystallization:

The crystallization may comprise adding a solubilizing agent to the positional isomer mixture resulting from the reduction; and adding a precipitating agent, and optionally filtering the precipitate; and concentrating the filtrate and adding an additional precipitating agent.

Examples of the solubilizing agent useful in the crystallization include acetone, acetonitrile, tetrahydrofuran, ethyl acetate, dichloromethane, chloroform, 1,4-dioxane, lower alcohol of 1 to 4 carbon atoms, and mixtures thereof, but are not limited thereto. The solubilizing agent may be added in an amount of zero to 20 ml (v/w) based on the weight (g) of the positional isomer mixture.

Non-limiting examples of the precipitating agent include water, a lower alcohol of 1 to 4 carbon atoms, diethylether, pentane, hexane, cyclohexane, heptane, and mixtures thereof. The precipitating agent may be slowly added in an amount of from zero to 40 ml (v/w) based on the weight (g) of the positional isomer mixture.

Following the addition of the precipitating agent, filtration may yield 1N alcohol (3a) as a precipitate of high purity.

Furthermore, 2N alcohol (3b) can be obtained as a crystal form of very high purity by concentrating the filtrate and increasing the ratio of the precipitating agent to the solubilizing agent.

These crystallization steps may be omitted when the positional isomers of arylketone of Chemical Formula 2 are already isolated and purified.

The introduction of a carbomoyl moiety into the alcohol compound with (R)-configuration of Chemical Formula 3 leads to carbamate with (R)-configuration, represented by Chemical Formula 1:

wherein,

R₁ and R₂ are independently selected from a group consisting of hydrogen, halogen, perfluoroalkyl, an alkyl of 1 to 8 carbon atoms, a thioalkoxy of 1 to 8 carbon atoms, and an alkoxy of 1 to 8 carbon atoms; and one of A₁ and A₂ is CFI with the other being N.

In the carbamation step, for example, inorganic cyanate-organic acid, isocyanate-water, or carbonyl compound-ammonia may be employed to introduce a carbamoyl moiety.

For the carbamation with inorganic cyanate-organic acid, the alcohol compound with (R)-configuration of Chemical Formula 3 is dissolved in an organic solvent, for example, diethylether, tetrahydrofuran, 1,4-dioxane, acetonitrile, dichloromethane, chloroform or mixtures thereof, and mixed with 1 to 4 equivalents of inorganic cyanate such as sodium cyanate and an organic acid, such as methane sulfonic acid or acetic acid, followed by reacting at about −10 to 70° C.

With regard to use of the isocyanate-water, 1 to 4 equivalents of isocyanate, for example, chlorosulfonic isocyanate, trichloroacetyl isocyanate, trimethylsilyl isocyanate, are added to a solution of the alcohol compound with (R)-configuration of Chemical Formula 3 in an organic solvent, for example, diethylether, tetrahydrofuran 1,4-dioxane, acetonitrile, dichloromethane, chloroform or mixtures thereof, and reacted at about −50 to 40° C. Subsequently, without purification, 1 to 20 equivalents of water are added to induce hydrolysis.

With regard to use of the carbonyl compound-ammonia, 1 to 4 equivalents of a carbonyl compound, for example, 1,1′-carbonyldiimidazole, carbamoly chloride, disuccinyl carbonate, phosgene, triphosgene, or chloroformate, are added to a solution of the alcohol compound with (R)-configuration of Chemical Formula 3 in an organic solvent, for example, diethylether, tetrahydrofuran, 1,4-dioxane, acetonitrile, dichloromethane, chloroform or mixtures thereof, and reacted at about −10 to 70° C. followed by adding 1 to 10 equivalents of ammonia without purification.

After the carbamation, the carbamate compound of Chemical Formula 1 thus obtained may be purified to higher optical and chemical purity through the following crystallization. The crystallization comprises adding a solubilizing agent to the product of the carbamation; and then adding a precipitating agent, and optionally filtering the precipitate and adding an additional precipitating agent. For pharmaceutical use, it is preferable that there is always a final purification of the carbamated product before use, but that there can be a crystallization step earlier in the process.

Non-limiting examples of the solubilizing agent include acetone, acetonitrile, tetrahydrofuran, ethyl acetate, dichloromethane, chloroform, 1,4-dioxane, lower alcohol of 1 to 4 carbon atoms, and mixtures thereof. Based on the weight (g) of the reaction product, the solubilizing, agent may be used in an amount of from zero to 20 ml (v/w).

Non-limiting examples of the precipitating agent include water, lower alcohols of 1 to 4 carbon atoms, diethylether, pentane, hexane, cyclohexane, heptane and mixtures thereof. Based on the weight (g) of the reaction product, the precipitating agent may be slowly added in an amount of from zero to 40 ml (v/w).

Comprising enantioselective enzymatic reduction, the method of the present invention can provide optically high pure carbamate compounds. In addition, the mild reaction conditions which the method of the present invention requires ensure process safety. Furthermore, the crystallization step applicable to large-scale production before or after the enantioselective enzymatic reduction or after the carbamation results in a higher chemical purity of the carbamate compounds. The carbamate compounds prepared according to the present invention are very useful in the treatment of CNS disorders such as convulsion.

A better understanding of the present invention may be obtained through the following examples which are set forth to illustrate, but are not to be construed as in any way limiting the present invention.

PREPARATION EXAMPLE 1 Preparation of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-1-yl)ethan-1-one

To a suspension of 2-bromo-2′-chloroacetophenone (228.3 g, 0.978 mol) and potassium carbonate (161.6 g, 1.170 mol) in acetonitrile (2000 mL) was added a 35 w/w % 1H-tetrazole dimethylformamide solution (215.1 g, 1.080 mol) at room temperature. These reactants were stirred for 2 h at 45° C. and distilled under reduced pressure to remove about 1500 mL of the solvent. The concentrate was diluted in ethyl acetate (2000 mL) and washed with 10% brine (3×2000 mL). The organic layer thus separated was distilled under reduced pressure to afford 216.4 g of an oily solid residue. To a solution of the solid residue in ethyl acetate (432 mL) was slowly added heptane (600 mL). The precipitate thus formed was filtered at room temperature and washed to yield 90.1 g (0.405 mol) of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-1-yl)ethan-1-one (hereinafter referred to as “1N ketone”).

¹H-NMR(CDCl₃)□8.87(s, 1H), d7.77(d, 1H),d 7.39-7.62(m, 3H),d 5.98(s, 2H)

PREPARATION EXAMPLE 2 Preparation of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-one

After the filtration of Preparation Example 1, the filtrate was concentrated and dissolved in isopropanol (100 mL), and to which heptane (400 mL) was then added to complete the crystallization. Filtering and washing at 5° C. afforded 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-one (hereinafter referred to as “2N ketone”) as a solid. 94.7 g (0.425 mol).

¹H-NMR(CDCl₃)d8.62(s, 1H), d7.72(d, 1H), d7.35-7.55(m, 3H), d6.17(s, 2H)

PREPARATION EXAMPLE 3 Preparation of Alcohol Compound of (R)-Configuration by Enantioselective Enzymatic Reduction via Various Oxidoreductases

The following four solutions were prepared as follows:

Enzyme Solution 1

Competent Escherichia coli StarBL21 (De3) cells (Invitrogen) were transformed with the expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 1. The Escherichia coli colonies transformed with the resulting expression constructs were then cultivated in 200 mL of LB medium (1% tryptone, 0.5% yeast and 1% sodium chloride) with 50 micrograms/mL of ampicillin or 40 micrograms/mL of kanamycin, respectively, until an optical density of 0.5, measured at 550 nm, was achieved. The expression of the desired recombinant protein was induced by the addition of isopropylthiogalactoside (IPTG) to a concentration of 0.1 mM. After 16 hours of induction at 25° C. and 220 rpm, the cells were harvested and frozen at −20° C. In the preparation of the enzyme solutions, 30 g of cells were resuspended in 150 mL of triethanolamine buffer (TEA 100 nM, 2 mM MgCl2 10% glycerol, pH 8) and homogenized in a high pressure homogenizer. The resultant enzyme solution was mixed with 150 mL glycerol and stored at −20° C.

Enzyme Solution 2

RB791 cells (E. coli genetic stock, Yale, USA) were transformed with the expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 2. The Escherichia coli colonies transformed with the resulting expression constructs were then cultivated in 200 mL of LB medium (1% tryptone, 0.5% yeast and 1% sodium chloride) with 50 micrograms/mL of ampicillin or 40 micrograms/mL of kanamycin, respectively, until an optical density of 0.5, measured at 550 nm, was achieved. The expression of the desired recombinant protein was induced by the addition of isopropylthiogalactoside (IPTG) to a concentration of 0.1 mM. After 16 hours of induction at 25° C. and 220 rpm, the cells were harvested and frozen at −20° C. In the preparation of the enzyme solutions, 30 g of cells were resuspended in 150 mL of triethanolamine buffer (TEA 100 nM, 2 mM MgCl2, 10% glycerol, pH 8) and homogenized in a high pressure homogenizer. The resultant enzyme solution was mixed with 150 mL glycerol and stored at −20° C.

Enzyme Solution 3

Enzyme solution 3 was prepared in the same manner as described in Enzyme solution 1 except that expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 3 instead of expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 1 was used.

Enzyme Solution 4

Enzyme solution 4 was prepared in the same manner as described for enzyme solution 2 except that expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 4 instead of expression constructs pET21-MIX coding for oxidoreductase SEQ ID NO 2 was used.

Different oxidoreductases contained in each of enzyme solutions 1 to 4 were examined as follows for the conversion of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-1-yl)ethan-1-one (1N ketone) and 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-one (2N ketone) to the corresponding 1(2-chlorophenyl)-2-(1,2,3,4-tetrazol-1-yl)ethan-1-ol (hereinafter, referred to as “1N alcohol”) and 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-ol (hereinafter, referred to as “2N alcohol”), respectively.

Reaction Batch A

160 μl buffer (TEA 100 nM, 2 mM MgCl2, 10% glycerol, pH 8) 100 μl NADPH (40 mg/ml) 40 μl 2-propanol 50 μl enzyme solution 1 2 mg 1N ketone or 2N ketone Reaction Batch B

160 μl buffer (TEA 100 nM, 2 mM MgCl2, 10% glycerol, pH 8) 100 μl NADPH (40 mg/ml) 40 μl 2-propanol 50 μl enzyme solution 2 2 mg 1N ketone or 2N ketone Reaction Batch C

350 μl buffer (TEA 100 nM, 2 mM MgCl2, 10% glycerol, pH 8) 0.05 mg NADP 50 μl enzyme solution 3 10 mg 1N ketone or 2N ketone 250 μl 4-methyl-2-pentanol 50 μl enzyme (oxidoreductase from Thermoanerobium brockii) solution for regeneration of cofactor Reaction Batch D

350 μl buffer (TEA 100 nM, 2 mM MgCl2, 10% glycerol, pH 8) 0.05 mg NADP 50 μl enzyme solution 4 10 mg 1N ketone or 2N ketone 250 μl 4-methyl-2-pentanol 50 μl enzyme (oxidoreductase from Thermoanerobium brockii) solution for regeneration of cofactor

After 24 h of incubating each reaction batch A, B, C and D, 1 mL of acetonitrile was added to each reaction batch which was centrifuged and transferred into a HPLC analysis vessel for enantiomeric excess and conversion. Conversion and ee-value of products are listed in Table 1 below calculated using the following equations: Conversion Rate (%)=[(Area of Product)/(Area of Reactant+Area of Product]×100 ee-value (%)=[(Area of R-Configuration−Area of S-Configuration)/(Area of R-Configuration+Area of S-Configuration)]×100

TABLE 1 ee-values Conversion % ee(enantiomer) (% of R-2N Reaction batch used reduced ketone) Alcohol, 2b R-1N Alcohol, 2a Reaction batch A >98 89(R) >99(R) Reaction batch B >98 >99(R)  >99(R) Reaction batch C >98 95(R) >99(R) Reaction batch D >98 98(R)  95(R)

PREPARATION EXAMPLE 4 Enzymatic Reduction via Oxidoreductase SEQ NO: 2

For the conversion of 1/N2N ketone to R-1N/R-2N alcohol, 30 μl of the enzyme solution 2 containing the oxidoreductase SEQ NO: 2 were added to a mixture of 300 μl of a buffer (100 mM TEA, pH 8, 1 mM MgCl2, 10% glycerol), 100 mg of a mixture of 1N ketone and 2N ketone (1N:2N=14%:86%), 0.04 mg NADP and 300 μl 2-butanol. The reaction mixture was incubated at room temperature under constant thorough mixing. After 48 hours, more than 98% of the ketones were reduced to an alcohol mixture of the following composition (R-2N alcohol 80%; S-2N alcohol 0%; R-1N alcohol 20%, S-1N alcohol 0%; 1N ketone 0%; 2N ketone 0%).

After general work up and recrystallization with ethyl acetatehexane, optically pure alcohols were obtained as below:

(R)-1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-1-yl)ethan-1-ol (1N alcohol)

¹H-NMR(CDCl₃) d8.74(s, 1H), d7.21-7.63(m, 4H), d5.57(m, 1H), d4.90(d, 1H), d4.50(d, 1H), d 3.18 (d, 1H).

(R)-1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-ol (2N alcohol)

¹H-NMR(CDCl₃) d8.55(s, 1H), d7.28-7.66(m, 4H), d5.73(d, 1H), d4.98(d, 1H), d4.83(d, 1H), d3.38(hr, 1H).

Preparation of Carbamate PREPARATION EXAMPLE 5 Preparation of Carbamic Acid (R)-1-(2-Chlorophenyl)-2-tetrazol-2-yl)ethyl ester

50 ml of the enzyme solution 2 containing the oxidoreductase SEQ NO: 2 were added to a mixture of 250 ml of a buffer (100 mM TEA, pH 8, 1 mM MgCl2, 10% glycerol), 50 g (225 mmol) of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-one (2N ketone), 4 mg NAD, 300 ml of 2-propanol and 150 mL of butyl acetate. The reaction mixture was stirred at room temperature. After 48 hours more than 98% of 2N ketone was reduced to corresponding (R)-1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-ol (R-2N alcohol) with >99% ee values. To this resulting mixture, 500 mL of ethyl acetate was added. After being separated, the organic layer thus formed was washed with 10% brine (3×500 mL). The organic layer thus formed was dried over magnesium sulfate and filtered and the filtrate was distilled under reduced pressure to give 50.4 g (224 mmol) of 1-(2-chlorophenyl)-2-(1,2,3,4-tetrazol-2-yl)ethan-1-ol (R-2N alcohol, optical purity 99.9%) as an oily residue. To this resulting crude product, 450 mL of tetrahydrofuran was added. After cooling to −15° C., 38 g (267 mmol) of chlorosulfonyl isocyanate was slowly added and stirred at −10° C. for 2 h. The slow addition of water induced termination of the reaction. The resulting solution was concentrated under reduced pressure until about 300 mL of the solvent was removed. The concentrate was diluted with 600 mL of ethyl acetate and washed with 10% brine (3×500 mL). The organic layer was concentrated under reduced pressure and the concentrate was dissolved in isopropanol (90 mL) to which heptane (180 mL) was slowly added, leading to the completion of crystallization. The precipitate thus obtained was filtered and washed to afford 51.8 g (194 mmol) of carbamic acid (R)-1-(2-chiorophenyl)-2-(tetrazol-2-yl)ethyl ester (optical purity 99.9%).

¹H-NMR(Acetone-d₆) d8.74(s, 1H), d7.38-7.54(m, 4H), d6.59(m, 1H), d6.16(Br, 2H), d4.90(d, 1H), d5.09(m, 2H)

As described, hitherto, carbamate compounds with high optical and chemical purity can be produced with an economical benefit in accordance with the present invention.

Although the preferred embodiments of the present invention have been disclosed for illustrative purposes, those skilled in the art will appreciate that various modifications, additions and substitutions are possible, without departing from the scope and spirit of the invention as disclosed in the accompanying claims.

Amino Acid Sequences

SEQ ID NO 1: Oryctolagus cuniculus from rabbit DSMZ 22167   1 massgvtrrd plankvaivt astdgiglai arrlaqdgah vvissrkqqn vdravaalqa  61 eglsvtgtvc hvgkaedrer lvatalnlhg gidilvsnaa vnpffgklmd vteevwdkil 121 dinvkamalm tkavvpemek rgggsvviva siaafnpfsg lgpynvskta lvgltknlal 181 elaaqnirvn clapglikts fskalwedka qeeniiqklr irrlgkpeec agivsflcse 241 dasyitgetv vvaggapsrl SEQ ID NO 2: Candida magnoliae DSMZ 22052 protein sequence carbonyl reductase   1 msatsnalit gasrgmgeat aiklalegys vtlasrgieq lnaikeklpi vkkgqqhyvw  61 qldlsdieaa stfkgaplpa ssydvffsna gvvdfapfad qsetaqkdlf tvnllspval 121 tktivkaiad kpretpahii ftssivgirg vpnvavysat kgaidsfars larefgpkni 181 hvncvnpgtt rtemtkgvdl aafgdvpikg wievdaiada vlflikskni tgqslvvdng 241 fgv SEQ ID NO 3: Candida vaccinii CBS7318 protein sequence carbonyl reductase   1 mrstpnalvt ggsrgigaaa aiklaeagys vtlasrgldk lnevkaklpv vkqgqehhvw  61 gldlsdvqaa lefkgaplpa skydlfvsna gvatfsptae hddkdwqnii avnltspiai 121 tkalvkavge rsndnpfqia flssaaalrg vpqtavysat kagldgftrs lakelgpkgi 181 hvnivhpgwt qtemtagvde prdtpipgwi gpeaiaeaiv ylaksknitg tnivvdnglt 241 i SEQ ID NO 4: Candida magnoliae CBS6396 protein sequence carbonyl reductase   1 mnalvtggsr gigeaiatkl aedgysvtia srgidqlnkv kaklpvvreg qthhvwqldl  61 sdaeaassfk gaplpassyd vlvnnagvtd pspiakqsds eihklfsvnl lspvaltkty 121 vqavtgkpre tpahiifiss gvairgypnv avysatksgl dgfmrslare lgpegvhvnt 181 vspgltktem asgvslddfp pspiggwiqp eaiadavryl vksknitgti lsvdngitv

Nucleic Acid Sequences

SEQ ID NO 5: Oryctolagus cuniculus from rabbit DSMZ 22167   1 atggcttcat ctggcgtaac acgccgtgat ccgctggcca acaaagtcgc tattgtcact  61 gcgtcgaccg atggcatcgg actggcgatt gcgcgtcgcc ttgctcagga cggggctcac 121 gtggtaatct cttcgcgtaa acagcaaaat gtagatcgtg ccgttgctgc cctgcaagca 181 gaaggtctgt ccgtaactgg tactgtgtgc catgtcggga aagccgagga ccgtgaacgt 241 ctggttgcga cggcccttaa tcttcatggc ggtatcgata tcctggtgag taacgcggcc 301 gtcaatccgt ttttcggtaa gttaatggac gtcaccgaag aggtgtggga taaaattctg 361 gacatcaacg tgaaagcaat ggcgttgatg accaaagcgg tggttccaga aatggaaaaa 421 cgcggtgggg gctcagttgt cattgtggcc agcattgcag cctttaatcc atttagcggc 481 ttaggtccgt acaatgtgag taaaacggca ttggttggcc tgaccaagaa cctggcattg 541 gagttagcag cgcagaacat tcgtgttaac tgtttagcgc cgggcctgat taagacatca 601 ttcagtaagg cactgtggga ggataaagct caggaggaaa atatcattca gaaactgcgt 661 attcgccgtc tgggaaaacc ggaagaatgt gcaggtatcg ttagctttct gtgctctgaa 721 gatgcgtcct atattacggg tgaaaccgta gtggttgccg gcggagcgcc gagccgcctg SEQ ID NO 6: Candida magnoliae DSMZ 22052 nucleic acid sequence carbonyl reductase   1 atgtctgcta cttcgaacgc tcttatcact ggtgccagcc gcggaatggg cgaggccaca  61 gctattaagc ttgcccttga ggggtacagc gtcacccttg catcacgcgg tattgagcag 121 ctcaatgcca tcaaggaaaa actacccatc gtgaagaagg gccagcagca ctacgtttgg 181 cagctcgatc ttagtgacat cgaggcggct tccaccttca agggggctcc tctgcctgcc 241 agcagctacg acgtgttctt cagcaacgcc ggtgtggtgg actttgctcc gttcgcagac 301 caaagcgaga ctgcgcaaaa ggacctgttc acggttaacc tgctgtcgcc tgttgcgttg 361 accaagacca ttgttaaggc catcgccgac aagccccgcg agacgcctgc tcacattatc 421 ttcacctcgt ccattgtcgg aattcgcggt gttcccaacg tggcggtcta cagcgccacc 481 aagggcgcga ttgacagctt tgcgcgctcg cttgctcgtg agttcggtcc caagaacatc 541 cacgttaact gcgtgaaccc gggcacgacg cgcaccgaga tgacaaaggg cgttgatctc 601 gcggctttcg gcgatgttcc tatcaagggc tggatcgagg tcgatgcgat tgccgacgct 661 gtgctgtttt tgatcaagtc caagaacatc actggccagt cgctcgttgt tgacaagcca 721 ttcggtgttt aa SEQ ID NO 7: Candida vaccinii CBS7318 nucleic acid sequence carbonyl reductase   1 atgaggtcga cacctaacgc ccttgtgact ggcggcagcc gcggcattgg cgcggccgct  61 gcaattaaac tcgccgaggc aggctacagc gtgacgctcg cgtcgcgcgg tctcgacaag 121 ctcaacgagg tgaaggccaa gcttcctgtc gtgaagcagg gccaggagca ccatgtatgg 181 cagcttgatc tcagcgacgt gcaggccgcg ctcgagttca agggcgcacc gctgcccgcg 241 agtaagtacg atttgtttgt ctcgaacgcc ggcgtggcta ctttctcgcc aacggctgag 301 catgacgaca aggactggca gaacattatt gccgtgaact tgacatcgcc cattgccatt 361 acgaaggcgc tcgttaaggc cgttggcgag cgctcaaacg ataacccgtt tcagatcgcg 421 ttcctgtcat cggcggccgc cctgcgcggt gtgccgcaga ccgctgttta cagcgctacg 481 aaggccggcc tcgacggctt cacgcgctcg ctcgccaagg agctcggccc aaagggcatc 541 catgtgaaca tcgtacaccc tggatggacg cagaccgaga tgactgcggg tgtagatgag 601 cctagggata cgcccatccc gggctggatc cagccggaag ccatcgccga ggccattgtg 661 tatctcgcga agtcaaagaa catcacggga acgaacatcg ttgtcgacaa cggcctgact 721 atttaa SEQ ID NO 8: Candida magnoliae CBS6396 nucleic acid sequence carbonyl reductase   1 atgaacgctc tagtgaccgg tggtagccgt ggcattggcg aggcgatcgc gaccaagctg  61 gccgaagatg gctacaccgt gacaatcgcc tcgcgcggaa tcgatcagct caacaaggta 121 aaggctaaac ttccggttgt gagggagggc cagacccacc acgtgtggca gcttgatttg 181 agcgacgccg aggccgcgtc gtccttcaag ggcgctcctt tgccagcaag cagctacgat 241 gtccttgtca acaacgccgg agtaacggat ccgagtccca ttgcgaagca gtcggatagc 301 gagattcaca agctgtttag cgtgaatctg ctgtcaccag ttgctttgac aaagacgtac 361 gtccaggcgg ttaccggaaa gcctcgtgag acgccagctc acattatttt tatctcgtca 421 ggcgttgcca ttcgaggcta cccaaacgtc gctgtatact cggctactaa gagcgggctc 481 gacggtttca tgaggtctct ggcgcgtgag cttggccccg agggcgtcca tgtgaacact 541 gtcagcttgg gtctcaccaa aaccgagatg gccagcggcg tcagccttga cgacttcccg 601 ccatcgccga ttgggggctg gatccagccc gaggccatcg ctgatgcagt gaggtacctg 661 gtgaagtcga agaacatcac aggcacgatt ctgtcagttg acaacggaat cacggtttaa 

What is claimed is:
 1. A method for preparing carbamic acid aryl-2-tetrazolyl ethyl ester of Chemical Formula 1, comprising: subjecting an arylketone of Chemical Formula 2 to enantioselective enzymatic reduction in a reaction mixture comprising said compound, an oxidoreductase having at least 90% homology with amino acid sequence SEQ ID NO: 1 or SEQ ID NO: 3, NADH or NADPH as a cofactor that is oxidized during the reduction process and continuously regenerated, a second substrate comprising a secondary alcohol having the Formula RR′CHOH, wherein R and R′ are independent from one another and have from 1 to 10 carbon atoms, and a suitable buffer to form an alcohol compound of (R)-configuration of Chemical Formula 3; and carbamating said alcohol,

 wherein R₁ and R₂ are independently selected from the group consisting of hydrogen, halogen, perfluoroalkyl, an alkyl of 1 to 8 carbon atoms, a thioalkoxy of 1 to 8 carbon atoms, and an alkoxy of 1 to 8 carbon atoms; and one of A₁ and A₂ is CH with the other being N.
 2. The method according to claim 1, wherein the oxidoreductase is encoded by nucleic acid sequence SEQ ID NO: 5 or SEQ ID NO:
 7. 3. The method according to claim 2, wherein the oxidoreductase is isolated from Candida magnolia, Candida vaccinii or Oryctolagus cuniculus.
 4. The method according to claim 1, wherein the oxidoreductase is purified or in a microbial cell.
 5. The method according to claim 1, wherein the oxidoreductase is partially purified.
 6. The method according to claim 1, wherein the oxidoreductase is a microbial cell lysate.
 7. The method according to claim 4, wherein the oxidoreductase is present in the microbial cells and is permeabilized.
 8. The method according to claim 7, wherein the microbial cells are transformed Escherichia coli cells.
 9. The method according to claim 1, wherein the oxidized cofactor is reduced to the cofactor by the oxidation of said second substrate.
 10. The method according to claim 1, wherein said second substrate is a secondary alcohol selected from the group consisting of 2-propanol, 2-butanol, 2-pentanol, 4-methyl-2-pentanol, 2-heptanol and 2-octanol.
 11. The method according to claim 1, wherein said oxidoreductase affects both the reduction of the arylketone of Chemical Formula 2 and the oxidation of the second substrate.
 12. The method according to claim 1, wherein the carbamating step comprises reacting the alcohol compound of (R)-configuration of Chemical Formula 3 with inorganic cyanate and an organic acid.
 13. The method according to claim 1, wherein the carbamating step comprises hydrolyzing a product resulting from reaction between the alcohol compound of (R)-configuration of Chemical Formula 3 and an isocyanate compound selected from the group consisting of chlorosulfonic isocyanate, trichloroacetyl isocyanate and trimethylsilyl isocyanate.
 14. The method according to claim 1, wherein the carbamating step comprises introducing ammonia into a product resulting from reaction between the alcohol compound of (R)-configuration of Chemical Formula 3 and a carbonyl compound comprising 1,1′-carbonyldiimidazole, carbamoylhalide, N,N-disuccinimidyl carbonate, phosgene, triphosgene or chloroformate.
 15. The method according to claim 1, further comprising crystallizing the compound of Chemical Formula
 1. 16. The method according to claim 15, wherein the crystallizing step comprises: adding to a reaction product a solubilizing agent selected from the group consisting of acetone, acetonitrile, tetrahydrofuran, ethyl acetate, dichloromethane, chloroform, 1,4-dioxane, an alcohol of 1 to 4 carbon atoms and mixtures thereof; and adding a precipitating agent thereto selected from the group consisting of water, an alcohol of 1 to 4 carbon atoms, diethylether, pentane, hexane, cyclohexane, heptane and mixtures thereof.
 17. The method according to claim 1, further comprising: preparing the arylketone of Chemical Formula 2 by a substitution reaction between an arylketone of Chemical Formula 4 with a tetrazole of Chemical Formula 5:

wherein R₁ and R₂ are as defined in claim 1; and X is a leaving group selected from the group consisting of halides and sulfonates.
 18. A method according to claim 17, further comprising a crystallizing step comprising: adding a solubilizing agent selected from the group consisting of acetone, acetonitrile, tetrahydrofuran, ethyl acetate, dichloromethane, chloroform, 1,4-dioxane, an alcohol of 1 to 4 carbon atoms and mixtures thereof to a product obtained by the substitution reaction; and adding a precipitating agent selected from the group consisting of water, an alcohol of 1 to 4 carbon atoms, diethylether, pentane, hexane, cyclohexane, heptanes and mixtures thereof.
 19. A method for preparing an alcohol compound of Chemical Formula 3, through the enantioselective enzymatic reduction of an arylketone of Chemical Formula 2:

wherein R₁ and R₂ are independently selected from the group consisting of hydrogen, halogen, perfluoroalkyl, an alkyl of 1 to 8 carbon atoms, a thioalkoxy of 1 to 8 carbon atoms, and an alkoxy of 1 to 8 carbon atoms; one of A₁ and A₂ is CH with the other being N; and said reduction is carried out in a reaction mixture comprising said compound of Chemical Formula 2, an oxidoreductase having at least 90% homology with amino acid sequence SEQ ID NO: 1 or SEQ ID NO: 3, NADH or NADPH as a cofactor that is oxidized during the reduction process and continuously regenerated, a second substrate comprising a secondary alcohol having the Formula RR′CHOH, wherein R and R′ are independent from one another and have from 1 to 10 carbon atoms, and a suitable buffer.
 20. The method according to claim 19, wherein the oxidoreductase is encoded by nucleic acid sequence SEQ ID NO: 5 or SEQ ID NO:
 7. 21. The method according to claim 19, wherein the oxidoreductase is isolated from Candida magnolia, Candida vaccinii or Oryctolagus cuniculus. 